Team:Lyon-INSA/notebook

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(Difference between revisions)
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<jour nb="13">
<jour nb="13">
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                         <date>Monday, 13th August:
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                         <date>Monday, August 13th 2012</date>
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For all :
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                        <title>For all purposes</title>
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- We identified the reason why the deletion of the site SpeI from pHT315 and pHT304 plasmids and filling-in was not successful: the Pfu enzyme needs Mg2+ and the buffer used did not contain any, so we decided to give it another try, this time with the proper buffer.
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<description>
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- The extracted plasmids containing the RFP gene in  the pSB1C3 backbone were digested and verified by electrophoresis.  
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<ul>
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Kill :
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<li>We identified the reason why the deletion of the site SpeI from pHT315 and pHT304 plasmids and filling-in was not successful : the Pfu enzyme requires Mg2+ and the buffer we used did not contain any, so we decided to give it another try, this time with the proper buffer.</li>
-
- Lysostaphin tests : Flasks of 25 mL of Bs 168 pWG 100 filtered supernatant are cultivated Friday and frozen at -20°C  Sunday (2 flasks of each). The control flask is filled with 25 mL of LB media.  These flasks are then frozen at -80°C and freeze-dried overnight.  
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<li>The extracted plasmids containing the RFP gene in  the pSB1C3 backbone were digested and verified by electrophoresis.</li>
-
- The gel electrophoresis of the digested plasmid Lysostaphin + Dispersin in pSB1C3 doesn’t correspond to the expected fragments. Similarly, the second electrophoresis shows that the clones with the constitutive promotor and Dispersin in pSB1C3 do not have the right plasmid : the digested fragments do not have  the right size.
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</ul>
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Surfactant :
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</description>
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- Transformation of the ligation sfp+abrB+pSB1A3 in the NM522 strain.
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                        <title>Kill</title>
 +
<description>
 +
<ul>
 +
<li>Lysostaphin tests : Flasks of 25 mL of Bs 168 pWG 100 filtered supernatant were cultivated Friday and frozen at -20°C  Sunday (2 flasks of each). The control flask is filled with 25 mL of LB media.  These flasks are then frozen at -80°C and freeze-dried overnight.</li>
 +
<li>The gel electrophoresis of the digested plasmid [Lysostaphin + Dispersin] in pSB1C3 doesn’t correspond to the expected fragments. Similarly, the second electrophoresis shows that the clones with [Constitutive promotor + Dispersin] in pSB1C3 do not have the right plasmid : the digested fragments do not have  the right size.</li>
 +
</ul>
 +
</description>
 +
                      <title>Surfactant</title>
 +
<description>
 +
Transformation of the ligation [sfp + abrB + pSB1A3] in the NM522 strain.
 +
</description>
 +
                      </jour>
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Tuesday, 14th August:
Tuesday, 14th August:

Revision as of 23:05, 9 September 2012


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